The GacS Sensor Kinase Regulates Alginate and Poly-beta -Hydroxybutyrate Production in Azotobacter vinelandii

doi:10.1128/JB.182.9.2624-2628.2000

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Journal of Bacteriology, May 2000, p. 2624-2628, Vol. 182, No. 9
0021-9193/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

The GacS Sensor Kinase Regulates Alginate and Poly- $beta$ -Hydroxybutyrate Production in Azotobacter vinelandii

Miguel Castañeda, Josefina Guzmán, Soledad Moreno, and Guadalupe Espín^*

Departamento de Microbiología Molecular, Instituto de Biotecnología, Universidad Nacional Autónoma de México, Cuernavaca Morelos 62250, México

Received 11 November 1999/Accepted 14 February 2000

	ABSTRACT

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Azotobacter vinelandii produces two polymers: the extracellular polysaccharide alginate and the intracellular polyester poly- $beta$ -hydroxybutyrate(PHB). A cosmid clone (pSMU588) from an A. vinelandii gene librarydiminished alginate production by A. vinelandii mucoid strainATCC 9046. The nucleotide sequence and predicted amino acid sequenceof the locus responsible for the mucoidy suppression revealed65% identity to Pseudomonas GacS, a transmembrane sensor kinaseof the two-component regulators, whose cognate response regulator,GacA, is a global activator regulating several products and virulencefactors. Plasmid pMC15, harboring gacS, and a strain carryinga gacS nonpolar mutation were constructed. Either pMC15 or thegacS mutation significantly reduced alginate production and transcriptionof algD, the gene coding for the key enzyme GDP-mannose dehydrogenaseof the alginate biosynthetic pathway. We found that the gacS mutationalso reduced PHB accumulation and impaired encystment. Taken together,these data indicate that in A. vinelandii the gacSA global systemregulates polymersynthesis.

	TEXT

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Azotobacter vinelandii is a nitrogen-fixing soil bacterium that undergoes differentiation to form desiccation-resistant cystsand produces two polymers of industrial importance: alginate andpoly- $beta$ -hydroxybutyrate (PHB). Both polymers are involved in theencystment process; alginate is a component of the cyst capsule(28), and PHB accumulation correlates with the frequency ofcyst formation (30).

A. vinelandii has been shown to possess an alginate biosynthetic gene cluster (2, 16, 20, 25, 32), organized inthree operons, one of which transcribes algD encoding a GDP-mannosedehydrogenase, which converts GDP-mannose to GDP-mannuronic acid,the substrate for alginate polymerization. The algUmucABCD clustercontrols alginate production. AlgU is a $sigma$ ^E homolog (19). The mucA and mucB genes code for negative regulatorsof AlgU activity. In strain ATCC 9046, transcription of the algDgene is initiated at three sites, one of which is AlgU dependent(2). AlgU activity was shown to be involved in the encystmentprocess independent of its role in alginate synthesis (23).

Three enzymes are involved in PHB biosynthesis in A. vinelandii: a $beta$ -ketothiolase, an acetoacetyl-coenzyme A reductase anda PHB synthetase (18). PHB synthesis in A. vinelandii was shownto be regulated at the level of the $beta$ -ketothiolase activity (18).The genes encoding the enzymes participating in PHB synthesisin A. vinelandii have not beenreported.

Members of our group have previously reported the identification of cosmid pSMU588 from a gene bank of nonmucoid strain UW136,which reduced alginate production in A. vinelandii ATCC 9046 (19).The characterization of pSMU588 reported here allowed us to identifya regulatory gene homologous to Pseudomonas gacS, coding for asensor kinase of the two-component regulatory systems. This studyalso provides evidence for GacS playing a role as a regulatorof alginate and PHB synthesis in A. vinelandii.

Identification of the locus responsible for the suppression of mucoidy. Mini-Tn5-lacZ1 (6) mutagenesis of plasmid pSMU588 was carried out to identify the locus responsible for the reduction ofalginate. A pSMU588::mini-Tn5-lacZ1 derivative that no longersuppressed mucoidy was isolated and named pSMU588-21. Alginateproduction of ATCC 9046 carrying this plasmid was determined andthe results are shown in Table 1.

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TABLE 1. Polymer production and encystment in A. vinelandii strains^a

We determined 3 kb of nucleotide sequence around the mini-Tn5-lacZ1 insertion. DNA sequence analysis revealed one open readingframe encoding a polypeptide of 905 amino acid residues, sharingsimilarity with transmembrane sensor kinases belonging to signaltransduction proteins of the family of two-component regulators(12). Among those with the highest identity (65%) was GacS (previouslycalled LemA), which is present in the following Pseudomonas species:P. syringae (13), P. viridiflava (15), P. fluorescens (5),P. aureofaciens (3), and P. tolaasii (11). In P. syringae,GacS and its cognate response regulator, GacA, are required forthe production of the toxin syringomycin and for extracellularproteases (27); in P. viridiflava, GacS controls protease, pectatelyase and alginate production (15); and in P. fluorecens, GacScontrols antibiotic production (5). A gacS homolog, rpfA, whichregulates the production of virulence factors, has been reportedin the phytopathogenic bacterium Erwinia carotovora (8). InP. aeruginosa and P. aureofaciens, GacA, the GacS cognate responseregulator, has been shown to be a global activator regulatingseveral products and virulence factors via acyl-L-homoserine lactones(3, 26).

The A. vinelandii GacS amino acid sequence contains specific motifs typical of the ArcB subfamily, histidine protein kinasesthat are characterized by containing, in addition to the two transmembranedomains and the orthodox transmitter H1 domain, a response regulatorD1 domain and a second phosphorylatable histidine, H2 (9, 14).The exact location of the mini-Tn5-lacZ1 mutation within gacSwas mapped between codons encoding amino acids 735 and736.

Plasmid pMC15. To rule out the possibility that plasmid pSMU588-21 no longer suppressed alginate production due to a polar effect of thegacS::mini-Tn5-lacZ1 insertion rather than to the lack of thegacS gene product, oligonucleotides gacS1 (5'-AAGCGGAGCTCGAGCCGTCAGG-3')and gacS2 (5'-ACGGTGCCGTCTCGAGTTTCCGCTC-3') were used to isolate,by PCR, a fragment containing the gacS gene flanked by the ATGcodon (200 bp upstream) and the stop codon (20 bp downstream);this fragment was cloned into plasmid pKT230 (1). The resultantplasmid, pMC15, was found to have a much stronger effect on alginateproduction (Table 1), confirming the negative effect of gacSon alginate production and ruling out the possibility of a polareffect.

Construction and characterization of gacS mutants. Sensor kinases of the two-component regulatory systems usually act as positive regulators by phosphorylating the cognate responseregulator. To investigate a positive role of gacS on alginatebiosynthesis, ATCC 9046 derivatives carrying gacS mutations wereconstructed: in A. vinelandii the insertion of $Omega$ cassettes intogenes with the same orientation as the direction of transcriptionproduces nonpolar mutations which allow transcription of the downstreamgenes in the same operon (21, 24). Plasmid pMC5, a pBluescriptKS(+) plasmid which carries a 2.5-kb SmaI DNA fragment includinggacS, was used to construct gacS:: $Omega$ -Sp mutations. A 2-kb fragmentcontaining a spectinomycin resistance gene ( $Omega$ -Sp) from plasmidpHP45 $Omega$ -Sp (7) was inserted into the unique EcoRI site presentwithin gacS. Plasmids pMC7 and pMC8 with the cassette insertedin both orientations were selected and introduced into strainATCC 9046. Sp^r transformants were selected. Strains JM1 and JM2 were isolatedand were shown, by Southern blot analysis, to carry the gacS:: $Omega$ -Spnonpolar and polar mutations, respectively (data not shown). RNAisolated from strains JM1, JM2, and ATCC 9046 were hybridizedwith a 700-bp fragment corresponding to the 3' end of gacS. Hybridizationof RNA from the wild type with that of the gacS nonpolar JM1 mutantbut not with that of the JM2 polar mutant was observed (data notshown). Both gacS mutant strains produced threefold less alginatethan the parental strain, ATCC 9046, when grown on solid medium(Table 1). When cultures of these mutants were grown on liquidmedium, a 30- to 60-fold reduction in alginate production wasdetected. These data indicate that the negative effect on alginateproduction observed is due to the lack of the gacS gene productand not to a polareffect.

GacS also controls PHB production. PHB granules were visible in cells of wild-type ATCC 9046 under a light microscope; however, no PHB granules were observedin cells of strains JM1 or JM2. PHB accumulation in these strainswas determined. As shown in Table 1, either a gacS mutation orplasmid pMC15 caused a significant reduction in PHB accumulation.Electron microscopic examination of cultures of ATCC 9046, JM2,and ATCC 9046/pMC15 was carried out as described previously (21),and the results are shown in Fig. 1. In contrast to the wild-typeATCC 9046, where big PHB granules are observed, strains JM2 andATCC 9046/pMC15 appear to contain numerous very small PHB granulesand disorganized or amorphic white structures that appear to containPHB. These observations indicate that GacS also regulates PHBaccumulation.

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FIG. 1. Electron micrographs of A. vinelandii cells grown for 48 h in Burk's medium supplemented with 2.0% sucrose. (A) Strain ATCC 9046; (B) strain JM2; (C) strain ATCC 9046/pMC15. Arrows indicate small PHB granules. Bars, 0.4 µm.

The effect of the gacS mutation on alginate and PHB production indicates that GacS plays a positive role in the regulationof polymer synthesis in A. vinelandii. This role is likely dueto the kinase activity of GacS that results in phosphorylationof GacA, leading to activation of alginate and PHB genes. On theother hand, in the presence of the gacS gene cloned into the pKT230vector, with a copy number of 15 to 20 (4), the synthesis ofthese polymers is significantly reduced. A similar observationwas reported for the Escherichia coli histidine protein kinaseRcsC, which, together with RcsA, positively regulates synthesisof colanic acid, a component of the capsule conferring resistanceto desiccation in E. coli (31). Cells carrying a multicopy rcsCplasmid were shown to reduce the level of colanic acid (10).However, the negative effects observed when two-component regulatorysystems are present on multicopy plasmids do not necessarily reflecta natural situation; thus, the reduced alginate level may representanartifact.

The algD gene is a target of signal transduction by GacS. algD, the gene encoding GDP-mannose dehydrogenase, the key enzyme in the alginate biosynthetic pathway, seems to be highlyregulated, since its transcription can initiate from three differentsites: p1, a $sigma$ ⁷⁰ type of promoter (2); p2, controlled by $sigma$ ^E (23); and p3. We determined whether the effect of GacS on alginatebiosynthesis was exerted on the transcription of the algD geneby measuring the $beta$ -galactosidase activity of strain WI12, an ATCC9046 derivative carrying an algD::lacZ gene fusion (in the presenceand absence of plasmid pMC15), as well as of strain WI12-1, aWI12 derivative carrying the gacS:: $Omega$ -Sp nonpolar mutation. The $beta$ -galactosidase activity was measured as reported by Miller (22);1 U corresonds to 1 nmol of O-nitrophenyl- $beta$ -D-galactoside hydrolyzedper min per µg of protein. Protein was determined by the Lowrymethod (17). All measurements were done in triplicate. The $beta$ -galactosidaseactivity was measured during growth on Burk's medium supplementedwith 2% sucrose (Fig. 2A). In both the WI12-1 and WI12/pMC15 strainsthe $beta$ -galactosidase activity was reduced (Fig. 2B). We determinedwhich of the algD promoters was regulated by GacS. Primer extensionof algD on RNA isolated from strains JM1 and ATCC 9046/pMC15 wasperformed as previously described (2). No primer extensionproducts were detected with RNA from these strains grown for 48h in liquid Burk's medium supplemented with 2% sucrose (Fig. 3).This result is in agreement with the low $beta$ -galactosidase activitylevel detected under the same conditions. These data show that,in regulating alginate synthesis GacS exerts influence on transcriptionof algD from its three promoters. Similarly, in Pseudomonas fluorecensGacS and GacA regulate gene expression by influencing the $sigma$ ^S levels in addition to being required for expression of genesnot regulated by $sigma$ ^S (33). Thus, the GacSA system controls expression from promotersrecognized by different sigma factors. In this regard, it is possiblethat the putative $sigma$ ⁷⁰ algD promoter, P1, may instead be a $sigma$ ^S-dependent promoter.

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FIG. 2. Growth (A) and $beta$ -galactosidase activity (B) on Burk's medium supplemented with 2% sucrose are shown for the strains WI12 (squares and black bars), WI12-1 (triangles and grey bars), and WI12/pMC15 (circles and white bars). Prot., protein.

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FIG. 3. Primer extension analysis of algD transcription. (A) DNA sequence of the 5' end of algD. Triangles indicate the start sites of algD transcription. The ATG initiation codon is overlined. (B) Primer extension of the algD gene in strains ATCC 9046 (lane 1), JM2 (lane 2), and ATCC 9046/pMC15 (lane 3).

GacA must mediate signal transduction between GacS and algD. Members of our group have identified in the A. vinelandii chromosomea gene homologous to gacA (M. Castañeda, J. Sánchez, and G.Espín, unpublished results). Whether GacA directly interactswith the algD promoter region remains to be determined. In P.aureofaciens, GacA functions upstream of the PhzR regulator, inthe signal transduction pathway that regulates antibiotic synthesisvia acyl-homoserine lactones (3); thus, it is possible thatin A. vinelandii other regulatory proteins mediate signal transductionbetween GacS, GacA, and algD.

It is difficult to speculate on the target of signal transduction by GacS in PHB synthesis, since regulation of the A. vinelandiiphb biosynthetic genes is presently unknown. The A. vinelandiigacS mutation caused a PHB leaky phenotype and affected the sizeof the PHB granules. Similarly, in Ralstonia eutropha, phaP, alocus causing a PHB leaky phenotype, encodes a PHB-binding proteinthat determines the size of polyhydroxyalkanoic acid granules(34). Thus, gacS could be involved in the control of a genehomologous to phaP.

Effect of the gacS mutation on encystment. Alginate has been shown to be essential for the formation of mature cysts (2). As shown above, strain JM1 produces somealginate on plates of Burk's medium supplemented with 2% sucrose,and strains producing similar or lower levels of alginate arestill able to form cysts (23); we analyzed the encysting capacityof strain JM1, measuring desiccation resistance of cultures inducedfor encystment as previously described (2). A reduction ofmore than 1,000-fold in encystment frequency was observed in thegacS mutant JM1 (Table 1). However under encysting conditions,i.e., in n-butanol plates, alginate production by strain JM1 wasvery low. Thus, as is the case with other mutants impaired inalginate production, strain JM1 is unable to form desiccation-resistantcysts. GacS may affect this differentiation process exclusivelyvia its effect on alginate biosynthesis; however, whether thisglobal regulator is required for expression of other genes involvedin encystment remains to beinvestigated.

Nucleotide sequence accession number. The nucleotide sequence determined in this study has the GenBank accession no. AF197912.

	ACKNOWLEDGMENTS

This work was supported by grant 27767 from CONACyT. M. Castañeda thanks CONACyT and PADEP-UNAM for financial support duringhis Ph.D.studies.

We thank G. Soberón, D. Segura, and C. Núñez for helpful discussions. We acknowledge R. Nájera for technicalsupport.

	FOOTNOTES

^* Corresponding author. Mailing address: Departamento de Microbiología Molecular, Instituto de Biotecnología, UniversidadNacional Autónoma de México, Apd. Postal 510-3, Cuernavaca Morelos62250, México. Phone: 52-73-291644. Fax: 52-73-172388. E-mail:espin{at}ibt.unam.mx.

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1.	Bagdasarian, M., R. Lurz, B. Ruckert, F. C. H. Franklin, M. M. Bagdasarian, J. Frey, and K. N. Timmis. 1981. Specific-purpose plasmid cloning vectors. II. Broad host range, high copy number, RSF1010-derived vectors, and a host-vector system for gene cloning in Pseudomonas. Gene 16:237-247[CrossRef][Medline].
2.	Campos, M. E., J. M. Martínez-Salazar, L. Lloret, S. Moreno, C. Núñez, G. Espín, and G. Soberón-Chávez. 1996. Characterization of the gene coding for GDP-mannose dehydrogenase (algD) from Azotobacter vinelandii. J. Bacteriol. 178:1793-1799[Abstract/Free Full Text].
3.	Chancey, S. T., D. W. Wood, and L. S. Pierson, III. 1999. Two-component transcriptional regulation of N-acyl-homoserine lactone production in Pseudomonas aureofaciens. Appl. Environ. Microbiol. 65:2294-2299[Abstract/Free Full Text].
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5.	Corbell, N., and J. E. Loper. 1995. A global regulator of secondary metabolite production in Pseudomonas fluorescens Pf5. J. Bacteriol. 177:6230-6236[Abstract/Free Full Text].
6.	De Lorenzo, V., M. Herrero, V. Jakubzik, and K. N. Timmis. 1990. Mini-Tn5 transposon derivatives for insertion mutagenesis, promoter probing, and chromosomal insertion of cloned DNA in gram-negative eubacteria. J. Bacteriol. 172:6568-6572[Abstract/Free Full Text].
7.	Fellay, R., J. Frey, and H. Krisch. 1987. Interposon mutagenesis of soil and water bacteria: a family of DNA fragments designed for in vitro insertional mutagenesis of gram-negative bacteria. Gene 52:147-154[CrossRef][Medline].
8.	Frederick, R. D., J. Chiu, J. L. Bennetzen, and A. K. Handa. 1997. Identification of a pathogenicity locus, rpfA, in Erwinia carotovora that encodes a two component sensor-regulator protein. Mol. Plant-Microbe Interact. 7:455-463.
9.	Georgellis, D., A. S. Linch, and E. C. C. Lin. 1997. In vitro phosphorylation study of the Arc two component system of Escherichia coli. J. Bacteriol. 179:5429-5435[Abstract/Free Full Text].
10.	Gervais, F. G., P. Phoenix, and G. R. Drapeau. 1992. The rcsB gene, a positive regulator of colanic acid biosynthesis in Escherichia coli, is also an activator of ftsZ expression. J. Bacteriol. 174:3964-3971[Abstract/Free Full Text].
11.	Han, B., P. Arnab, and K. Johnstone. 1997. Spontaneous duplication of 661 bp element within a two component sensor regulator gene causes phenotypic switching in colonies of Pseudomonas tolaasii, cause of brown blotch disease of mushrooms. Mol. Microbiol. 25:211-218[CrossRef][Medline].
12.	Hoch, J. A., and T. J. Silhavy (ed.). 1995. Two-component signal transduction. American Society for Microbiology, Washington, D.C.
13.	Hrabak, E. M., and D. K. Willis. 1992. The lemA gene required for pathogenicity of Pseudomonas syringae pv. syringae on bean is a member of a family of two-component regulators. J. Bacteriol. 174:3011-3020[Abstract/Free Full Text].
14.	Ishige, K., S. Nagasawa, S. Tokishita, and T. Mizuno. 1994. A novel device of bacterial signal transducers. EMBO J. 13:5195-5202[Medline].
15.	Liao, C. H., D. E. MacCullus, and W. F. Fett. 1994. Molecular characterization of two gene loci required for production of the key pathogenicity factor pectate lyase in Pseudomonas viridiflava. Mol. Plant-Microbe Interact. 7:391-400[Medline].
16.	LLoret, L., R. Barreto, R. León, S. Moreno, J. Martínez-Salazar, G. Espín, and G. Soberón-Chávez. 1996. Genetic analysis of the transcriptional arrangement of Azotobacter vinelandii alginate biosynthetic genes: identification of two independent promoters. Mol. Microbiol. 21:449-457[CrossRef][Medline].
17.	Lowry, O. H., N. J. Rosebrough, A. L. Farr, and J. Randall. 1951. Protein measurement with the Folin phenol reagent. J. Biol. Chem. 193:265-275[Free Full Text].
18.	Manchak, J., and W. J. Page. 1994. Control of polyhydroxyalkanoate synthesis in Azotobacter vinelandii strain UWD. Microbiology 140:953-963[Abstract/Free Full Text].
19.	Martínez-Salazar, J. M., S. Moreno, R. Nájera, J. C. Boucher, G. Espín, G. Soberón-Chávez, and V. Deretic. 1996. Characterization of the genes coding for the putative sigma factor AlgU and its regulators MucA, MucB, MucC, and MucD in Azotobacter vinelandii and evaluation of their roles in alginate biosynthesis. J. Bacteriol. 178:1800-1808[Abstract/Free Full Text].
20.	Mejía-Ruíz, H., J. Guzmán, S. Moreno, G. Soberón-Chávez, and G. Espín. 1997. The Azotobacter vinelandii alg8 and alg44 genes are essential for alginate synthesis and can be transcribed from an algD-independent promoter. Gene 199:271-277[CrossRef][Medline].
21.	Mejía-Ruíz, H., S. Moreno, J. Guzmán, R. Nájera, R. León, G. Soberón-Chávez, and G. Espín. 1997. Isolation and characterization of an Azotobacter vinelandii algK mutant. FEMS Microbiol. Lett. 156:101-106[Medline].
22.	Miller, J. H. 1972. Experiments in molecular genetics, p. 431-435. Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.
23.	Moreno, S., J. Guzmán, R. Nájera, G. Soberón-Chávez, and G. Espín. 1998. Role of the alternative $sigma$ factor AlgU in encystment of Azotobacter vinelandii. J. Bacteriol. 180:2766-2769[Abstract/Free Full Text].
24.	Mouncey, N. J., L. A. Mitchell, and R. Pau. 1995. Mutational analysis of genes of the mod locus involved in molybdenum transport, homeostasis, and processing in Azotobacter vinelandii. J. Bacteriol. 177:5294-5302[Abstract/Free Full Text].
25.	Rehm, H. A., H. Ertesvag, and S. Valla. 1996. A new A. vinelandii mannuronan C-5 epimerase gene (algG) is part of an alg gene cluster physically organized in a manner similar to that in P. aeruginosa. J. Bacteriol. 178:5884-5889[Abstract/Free Full Text].
26.	Reimmann, C., M. Beyeler, A. Latifi, H. Winteler, M. Foglino, A. Lazdunski, and D. Haas. 1997. The global activator GacA of Pseudomonas aeruginosa PAO positively controls the production of the autoinducer N-butyryl-homoserine lactone and the formation of the virulence factors pyocyanin, cyanide, and lipase. Mol. Microbiol. 24:309-319[CrossRef][Medline].
27.	Rich, J. J., T. G. Kinscherf, T. Kitten, and D. K. Willis. 1994. Genetic evidence that the gacA gene encodes the cognate response regulator for the lemA sensor in Pseudomonas syringae. J. Bacteriol. 176:7468-7475[Abstract/Free Full Text].
28.	Sadoff, H. L. 1975. Encystment and germination in Azotobacter vinelandii. Bacteriol. Rev. 39:516-539[Free Full Text].
29.	Segura, D., and G. Espín. 1998. Mutational inactivation of a gene homologous to Escherichia coli ptsP affects poly- $beta$ -hydroxybutyrate accumulation and nitrogen fixation in Azotobacter vinelandii. J. Bacteriol. 180:4790-4798[Abstract/Free Full Text].
30.	Stevenson, L. H., and M. D. Socolofsky. 1966. Cyst formation and poly-hydroxybutyric acid accumulation in Azotobacter. J. Bacteriol. 91:304-310[Abstract/Free Full Text].
31.	Stout, V., and S. Gottesman. 1990. RcsB and RcsC: a two-component regulator of capsule synthesis in Escherichia coli. J. Bacteriol. 172:659-669[Abstract/Free Full Text].
32.	Vázquez, A., S. Moreno, J. Guzmán, A. Alvarado, and G. Espín. 1999. Transcriptional organization of the Azotobacter vinelandii algGXLIVFA genes: characterization of algF mutants. Gene 232:217-222[CrossRef][Medline].
33.	Whistler, C. A., N. A. Corbell, A. Sarniguet, W. Ream, and J. E. Loper. 1998. The two component regulators GacS and GacA influence accumulation of the stationary-phase sigma factor sigmaS and the stress response in Pseudomonas fluorescens Pf-5. J. Bacteriol. 180:6635-6641[Abstract/Free Full Text].
34.	Wieczorek, R., A. Pries, A. Steinbüchel, and F. Mayer. 1995. Analysis of a 24-kilodalton protein associated with the polyhydroxyalkanoic acid granules in Alcaligenes eutrophus. J. Bacteriol. 177:2425-2435[Abstract/Free Full Text].

The GacS Sensor Kinase Regulates Alginate and Poly--Hydroxybutyrate Production in Azotobacter vinelandii

The GacS Sensor Kinase Regulates Alginate and Poly- $beta$ -Hydroxybutyrate Production in Azotobacter vinelandii